Cloning of novel soluble gp130 and detection of its neutralizing autoantibodies in rheumatoid arthritis
Masao Tanaka, … , Masao Murakami, Kazuwa Nakao
Masao Tanaka, … , Masao Murakami, Kazuwa Nakao
Published January 1, 2000
Citation Information: J Clin Invest. 2000;106(1):137-144. https://doi.org/10.1172/JCI7479.
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Article

Cloning of novel soluble gp130 and detection of its neutralizing autoantibodies in rheumatoid arthritis

Abstract

In an attempt to isolate disease-associated autoantigens in rheumatoid arthritis (RA), we cloned a new autoantigen named gp130-RAPS, which is a novel soluble form of the IL-6 signal–transducing molecule gp130. gp130-RAPS is a 50-kDa protein translated from alternatively spliced mRNA and has a truncated form of gp130 with a unique sequence, Asn-Ile-Ala-Ser-Phe (NIASF), in its COOH-terminus. We observed serum antibodies to this NIASF sequence frequently in patients with RA, but not in those with other systemic rheumatic diseases or in healthy subjects. In RA, detection of those antibodies was significantly associated with disease activity indices such as serum C–reactive protein (CRP) levels, erythrocyte sedimentation rate, blood platelet counts, and serum IL-6 concentration. In vitro experiments revealed that gp130-RAPS inhibited IL-6 activity, and this inhibition was neutralized by antibodies to the COOH-terminus of gp130-RAPS derived from patients with RA. Thus, autoantibody to gp130-RAPS may play an important role in the progression of RA by promoting IL-6 activity. Inspection of autoantibodies to gp130-RAPS may become a practical clinical test for RA. gp130-RAPS and its autoantibody provide a new clue to the complicated pathogenesis of RA.

Authors

Masao Tanaka, Masaaki Kishimura, Shoichi Ozaki, Fumio Osakada, Hidetaka Hashimoto, Mitsuo Okubo, Masao Murakami, Kazuwa Nakao

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Competitive ELISA for fine epitope analysis. ELISA was performed with se...
Competitive ELISA for fine epitope analysis. ELISA was performed with sera from three patients with RA (RA1, RA2, and RA3) whose titers of α-RAPC15 Ab’s were 100, 37.2, and 9.6 U/mL, respectively. Competitor peptide 1 is control peptide RAPC15. Peptides with 10–amino acid sequences in RAPC15 where isoleucine 326 or COOH-terminal phenylalanine 329 was replaced with glycine or removed (peptides 3, 5, and 8) exhibited no significant inhibition (< 25%). Glycine 9 mer bearing COOH-terminal phenylalanine (peptide 10) showed little inhibition. Percent inhibition values were calculated with the formula: (OD [nonabsorbed sera] – OD [sera absorbed by competitor peptides]) / OD [nonabsorbed sera] × 100.